P. yezoensis was obtained from Myeongji (Busan, Korea) and stored at −70°C. The frozen samples were lyophilized and homogenized prior to protein extraction. The crude soluble fraction was extracted with 0.1 M sodium acetate buffer (pH 6.0). Samples of P. yezoensis (1 g) were mixed with 50 ml sodium acetate buffer for 16 h with continuous shaking at 4°C, and then filtered through Whatman No. 1 filter paper. The extract was then precipitated with methanol and chloroform (28). Protein material was precipitated to increase the purity and the resulting supernatants were treated with a 2-D Clean-up kit (GE Healthcare Life Sciences, Logan, UT, USA). Protein concentrations were determined using a bicinchoninic acid assay with bovine serum albumin (Thermo Fisher Scientific, Inc., Waltham, MA, USA) as the standard.

For 2D-PAGE analysis, isoelectric focusing was performed as the first dimension and SDS-PAGE as the second dimension, according to the manufacturer's protocols (GE Healthcare Life Sciences). Protein samples (150 µg) containing 0.5% immobilized pH gradient (IPG) buffer (pH 4-7) and 5% bromophenol blue were applied to an immobilized IPG DryStrip (pH 4-7, 13 cm, GE Healthcare Life Sciences) and rehydrated for 16 h in lysis solution containing 4 M urea, 4% 3-(3-cholami-dopropyl dimethylammonio) propanesulfonate, 2 M thiourea, 100 mM dithiothreitol and 1% polyvinylpyrrolidone. Prior to performing the second dimension SDS-PAGE, focused IPG strips were equilibrated for 20 min in a solution of 50 mM Tris-HCl (pH 8.8), 6 M urea, 30% glycerol, 2% SDS and 1% DTT, and then for an additional 20 min in the same solution, but with the DTT replaced with 0.5% iodoacetamide. The equilibrated strips were positioned on a 15% polyacrylamide gel (14×13 cm, 1.5 mm) and, following SDS-PAGE the gels were silver-stained. Analysis of the partial amino acid sequences of the soluble proteins was performed using electrospray ionization quadrupole time-of-flight mass spectrometry/mass spectrometry (ESI Q TOF MS/MS), as described previously (29).

The P. yezoensis PBP-derived peptides (PBP 1-13) were synthesized by Peptron (Daejeon, Korea). Purification of the 13 peptides was performed on a C18 column (Shiseido CAPCELL PAK; Shiseido, Tokyo, Japan) attached to a high-performance liquid chromatography apparatus with elution in 0.1% trifluoroacetic acid and a gradient of 3-70% acetonitrile, a flow rate of 1 ml/min and UV detection at 220 nm. The peptide molecular weights, as shown in Table I, were determined by mass analysis (HP 1100 series LC/MSD; Agilent Technologies, Inc., Santa Clara, CA, USA).

The HepG2 human hepatoblastoma cell lines were obtained from American Type Culture Collection (Rockville, MD, USA). The cells were cultured at 37°C in a humidified 5% CO₂, 95% air equilibrated incubator in modified Eagle's medium (Sigma-Aldrich; Merck KGaA, Darmstadt, Germany) supplemented with heat-inactivated 10% fetal bovine serum (FBS; HyClone, Logan, UT, USA), 100 U/ml penicillin and 100 µg/ml streptomycin. The adherent cells were detached with trypsin-EDTA solution and plated at 70-80% confluence.

Cell viability was measured with fluorescein diacetate (FDA) and propidium iodide (PI), which stain viable cells and dead cells, respectively. The cells were seeded at a density of 1.5×10⁴ cells per well in a 96-well plate. PBP 1-13 (1 µg/ml) were added and the cells were treated with 5 mM H₂O₂ for 1 h. The cell culture medium was then removed and FDA (at a final concentration of 10 µg/ml) or PI (at a final concentration of 5 µg/ml) was added. The cells were incubated at 37°C for 30 min. The staining solutions were removed and the samples were washed with phosphate-buffered saline (PBS). In order to determine the experimental concentrations of PBP peptides, a preliminary experiment was performed using 1-100 µg/ml of peptides with FDA and PI. The subsequent experiments were performed using the range of 0.001-0.01-0.1-1 µg/ml, which showed the concentration-dependent changes and suitability in measurement (data not shown).

Inhibition of ROS production by PBP 1-13 was evaluated in the HepG2 cells using a cell permeable probe, 2′,7′-dichlorofluorescein diacetate (DCF-DA). The cells were seeded onto 96-well plates (1.5×10⁴ cells per well), grown until confluence and pre-incubated with 50 µM DCF-DA for 1 h at 37°C in the dark. Following washing with PBS away excess probe, the cells were treated with PBS or PBP 1-13 (1 µg/ml) in the presence or absence of 5 mM H₂O₂, for 1 h. Ascorbic acid (1 µg/ml) was used as an antioxidant control.

Fluorescence was measured using a FilterMax F5 Multi-Mode microplate reader (Molecular Devices LLC, Sunnyvale, CA, USA) and an Epi-fluorescence microscope (Nikon Corporation, Tokyo, Japan) with the following settings: Excitation 485 nm and emission 535 nm for FDA and DCF-DA, and excitation 535 nm and emission 615 nm for PI. The viability and ROS production of the synthetic peptide-treated cells were calculated as a percentage of that in the untreated control cells.

Quantitative analysis of living and dead cells according to PBP2 concentrations were performed according to the manufacturer's protocol of the FITC Annexin V Apoptosis Detection Kit I (BD Biosciences, Franklin Lakes, NJ, USA) and measured with a Muse™ Cell Analyzer (EMD Millipore, Billerica, MA, USA). To measure the number of stained cells, ImageJ software (version 1.41; National Institutes of Health, Bethesda, MD, USA) was used alongside Cell Counting Macro 1 [version 1.0; developed by Kurt De Vos (Academic Neurology, University of Sheffield, Shefield, UK) and used by the GNU General Public License, https://github.com/grishagin/CellCounting/archive/master.zip].

The cells were seeded at a density of 1.5×10⁴ cells per well in a 96-well plate. PBP2 (1 µg/ml) was added and the cells were treated with 5 mM H₂O₂ for 1 h. The cell culture medium was then removed, and the cells were washed with PBS. The cells were then stained with Annexin V and PI for 15 min in the dark at 25°C.

Whole cell extracts for the detection of SOD, CAT and GPx by immunoblotting were isolated from the H₂O₂-treated HepG2 cells with or without PBP 1-13 peptide treatment. Separation of nuclei was performed using the Nuclei EZ Prep nuclear isolation kit (Sigma-Aldrich; Merck KGaA, Darmstadt, Germany) according to the manufacturer's protocols. Protein concentration was determined by bicinchoninic acid assay. The cell lysates (30 µg) and nuclei (20 µg) were separated by electrophoresis on a 15% SDS-PAGE gel and transferred onto polyvinylidene difluoride membranes (EMD Millipore) using a semi-dry transfer system. The membranes were blocked with 1% BSA in TBST buffer (0.1% Tween 20 in TBS) overnight at 4°C and incubated with the following primary antibodies: SOD2 (1:2,000; cat. no. OASE00357; Aviva Systems Biology, San Diego, CA, USA), CAT (1:500; cat. no. OAAB05216; Aviva Systems Biology), GPx1 (1:1,000; cat. no. OAAF05777; Aviva Systems Biology), PCNA (1:1,000; cat. no. sc-56, Santa Cruz Biotechnology, Inc., Heidelberg, Germany), β-actin (1:1,000; cat. no. sc-47778; Santa Cruz Biotechnology Inc.), nuclear factor erythroid-derived 2-like 2 (Nrf2; 1:1,000; cat. no. sc-722; Santa Cruz Biotechnology, Inc.); p-Nrf2 (1:5,000; cat. no. ab76026; Abcam, Cambridge, UK) in TBST solution containing 1% BSA for 1 h at room temperature. Following washing three times with TBST, the membranes were incubated for 1 h at room temperature with anti-rabbit and anti-mouse secondary antibodies (Thermo Fisher Scientific, Inc.) with horseradish peroxidase and washed with TBST three times. The final detection was performed with enhanced chemiluminescence western blotting reagents (Santa Cruz Biotechnology, Inc.). GeneTools software (version 4.03; Syngene, Cambridge, UK) was used for densitometry.

Data are expressed as the mean ± standard deviation and were evaluated by one-way analysis of variance using the statistical package for social sciences version 10.0 (SPSS, Inc., Chicago, IL, USA). Values were compared with controls using one-way analysis of variance followed by Duncan's multiple range tests. P<0.05 was considered to indicate a statistically significant difference.

Soluble proteins were extracted from P. yezoensis and separated by 2D-PAGE. The soluble proteins were classified by their isoelectric points (pIs) using a strip with a pH range of 4-7. As shown in Fig. 1, ~200 spots were resolved. To characterize PBPs with pI values of 4-6, 60 spots observed between 11 and 25 kDa were analyzed by ESI-Q TOF MS/MS. As a result, 10 spots were identified as PBPs (enclosed with circles in the tetragon in Fig. 1A). As shown in Table I, the identified PBPs were PE (spots 42, 43, 51, 52 and 54), PC (spots 61 and 59) and APC (spots 47, 48 and 49). PE was identified as the α-type based on peptide sequences analyzed from spots 51, 52 and 54, RFP SSS DLE SVQ GNI QRA, RTL NLP TSA YVA SFA FAR D and KSV ITT TIS AAD AAG RFP SSS DLE SVQ GNI QRA; and as the β-type based on sequences from spots 42, 43 (Fig. 1B and C), 51 and 52, KAA AVA FIT NTA SQR K and RYV SYA LLA GDP SVL EDR C. PC was identified as the α-type with the sequences analyzed from spots 61 and 69, RFL SNG ELQ AIN GRY, RLI TGA AQS VYT KF, KTP ITE AIA SAD SQG RF and KFP YVT QMP GPT YAS SAI GKA. APC-α was identified by the sequences of spots 47 and 48, MQD AIT SVI NAA DVQ GKY, RAA ATI AAN AAT IIK E and RYA TYG MLA GDP SIL EER V, whereas APC-β was identified by the sequence of spot 49, RLV TYG IVA GDV TPI EEI GLV GVK E.

The HepG2 human hepatoblastoma cell line derived from the HepG2 cell line can be used for investigations of xenobiotic metabolism as it maintains the synthesis and secretion of plasma proteins and cell surface receptors, which are specific functions of normal liver parenchymal cells (18,19). This was performed in the present study to confirm the protective effect of PBP peptides on oxidative stress and liver injury induced by the H₂O₂ in vitro system. As the liver is central for detoxification in vivo, HepG2 cell line, which is a human liver cell, was used as a target to observe the protective effect of oxidative stress.

The synthetic peptides, listed in Table I, were administered at 1 µg/ml to the HepG2 human liver cells, and their viabilities and ROS inhibition activities were determined. The fluorescent indicator dyes DCF-DA, FAD and PI load readily into guard cells, and their optical properties make them amenable to analysis using a fluorescence spectrophotometer. As shown in Fig. 2A, the number of viable cells was reduced to 47% by 5 mM H₂O₂. PBP1, 2 and 7-9 increased the number of viable cells by 23-32%, whereas dead cells stained with PI increased 2.3-fold by 5 mM H₂O₂ (Fig. 2B). PBP 1-13 reduced dead cells by 30-143%. In particular, PBP2 decreased to the negative control level. The ratio of viable cells to dead cells was reduced to 0.23 by 5 mM H₂O₂, but recovered in the presence of PBP1-4, 7-9 and 12 (Fig. 2C). In particular, PBP1-2 led to recovery with a ratio over three times higher than that of the positive control. Treatment with 5 mM H₂O₂ increased the production of ROS ~2-fold compared with that of the negative control (Fig. 2D). PBP 1, 2, 7-9 and 11-13 led to a 17-56% reduction in the production of ROS compared with that of the positive control. As a result, PBP 1, 2, 7-9 and 12 protected cells from oxidative stress by H₂O₂ and exhibited an antioxidative effect.

In particular, PBP2 showed good efficacy in terms of cell survival, prevention of death and inhibition of ROS production compared with 1 µg/ml ascorbic acid, a well-known antioxidant.

The HepG2 cells were stained with DCF-DA, PI, Annexin V and FDA, and observed with a fluorescence microscope and a fluorescence absorbance spectrophotometer to determine cytoprotective activity and antioxidant activity according to the concentration of PBP2 (0.001-1 µg/ml). The viable cell number decreased in the presence of 5 mM H₂O₂, whereas the number of dead cells and ROS increased (Fig. 3A and B). PBP2 at concentrations of 1 µg/ml increased the number of living cells and restored apoptotic cells and dead cells to negative control levels. In addition, 0.1-1 µg/ml PBP2 reduced the production of ROS by >50% when compared with that of the positive control.

To examine the possible mechanisms underlying the antioxidative effect, the present study investigated the effects of 1 µg/ml PBP2 on the p-Nrf2/antioxidant enzyme (CAT, SOD and GPx) pathway in HepG2 cells. As shown in Fig. 4A and B, HepG2 cells exposed to 5 mM H₂O₂ showed a significant decrease in the level of p-Nrf2. However, a marked increase in the level of p-Nrf2 was detected in the 0.1-1 µg/ml PBP2-treated groups. The expression levels of CAT and GPX were not significantly affected by 5 mM H₂O₂, however, SOD was decreased by 5 mM H₂O₂ and increased by treatment with PBP2 (Fig. 4C and D). GPX was not affected by 5 mM H₂O₂, but was increased by the effect of PBP2, suggesting that it was used to reduce the increased ROS. This increase was not concentration-dependent in the range of 0.01-1 µg/ml, suggesting that the removal of ROS used antioxidant enzymes other than SOD and GPX. The present study did not examine all the antioxidant enzymes and mechanisms, but confirmed the possibility. Therefore, the results of the present study may assist in elucidating the more specific mechanism of PBP2.

The results showed that treatment with 5 mM H₂O₂ led to decreases in the expression of p-Nrf2 and SOD, which were reversed by treatment with 0.1-1 µg/ml PBP2. However, no significant difference in the protein level of CAT was observed among these groups. These data suggested that PBP2 controlled H₂O₂-induced oxidative stress by regulating the expression of p-Nrf2/SOD.